Impact of Sample Preparation Methods on Single-Cell X-ray Microscopy and Light Elemental Analysis Evaluated by Combined Low Energy X-ray Fluorescence, STXM and AFM

Background: Although X-ray fluorescence microscopy is becoming a widely used technique for single-cell analysis, sample preparation for this microscopy remains one of the main challenges in obtaining optimal conditions for the measurements in the X-ray regime. The information available to researchers on sample treatment is inadequate and unclear, sometimes leading to wasted time and jeopardizing the experiment’s success. Many cell fixation methods have been described, but none of them have been systematically tested and declared the most suitable for synchrotron X-ray microscopy. Methods: The HEC-1-A endometrial cells, human spermatozoa, and human embryonic kidney (HEK-293) cells were fixed with organic solvents and cross-linking methods: 70% ethanol, 3.7%, and 2% paraformaldehyde; in addition, HEK-293 cells were subjected to methanol/ C3H6O treatment and cryofixation. Fixation methods were compared by coupling low-energy X-ray fluorescence with scanning transmission X-ray microscopy and atomic force microscopy. Results: Organic solvents lead to greater dehydration of cells, which has the most significant effect on the distribution and depletion of diffusion elements. Paraformaldehyde provides robust and reproducible data. Finally, the cryofixed cells provide the best morphology and element content results. Conclusion: Although cryofixation seems to be the most appropriate method as it allows for keeping cells closer to physiological conditions, it has some technical limitations. Paraformaldehyde, when used at the average concentration of 3.7%, is also an excellent alternative for X-ray microscopy.


Introduction
X-ray fluorescence (XRF) microscopy is a valuable technique for studying biological samples [1] because it provides the distribution of elements in tissues and cells nondestructively, without the need for stains or fluorescent probes. Mapping the distribution and content of endogenous and exogenous elements and metals is pivotal, especially for those elements with great biological importance, named also as "life elements" [2]. In addition, the ability to map samples at the nanometre scale provides the opportunity fixative-free samples. In cryofixation, the sample must be frozen fast enough for the water to change from its normal liquid state to its solid state (vitrification) without an ice crystal phase in between. Ice has a larger volume than water and can therefore cause deformation of the biological ultrastructure. While a variety of samples are suitable for rapid freezing, only a small volume of the sample will produce amorphous (ice-crystal free) ice. Viruses, proteins, organelles, and cells can be quickly iced; however, their volume makes tissues and multicellular organisms much more challenging to be properly cryofixated. Some experimental set-ups enable investigating frozen cells in a frozen hydrated state, under cooling [16]. Even if this condition allows for better sample preservation and reduces radiation damage effects, it requires a complex cryo-stage and cryo-transfer of the samples, which are not available in all facilities, making the experiments much more difficult starting from the sample preparation step till the final analysis [17].
Finally, sample preparation seems to influence the extent of radiation damage caused by soft X-rays during analyses [18][19][20]; therefore, this effect should also be taken into consideration during the selection of the ideal sample preparation.
In summary, the information available to researchers on sample treatment is still insufficient and sometimes ambiguous, leading to the uncertain success of the experiment.
In this study, we combined XRFM with atomic force microscopy (AFM) to evaluate how different fixatives can alter and influence the content and distribution of light chemical elements, diffusible ions, and cell morphology. The comparison will provide helpful information for synchrotron scientists to determine the most appropriate protocol for a particular study or cell model.
As cell models, we have chosen (i) the human HEC-1-A adenocarcinoma endometrial cell line as a model of an adherent immortalised tumour cell line, (ii) human spermatozoa as an example of primary suspension cells, and (iii) the immortalised human embryonic 293 cell line (HEK-293), which are genetically identical cells, thus ensuring repeatability of the experiments. As fixation methods, we have selected (i) 70% ethanol (EtOH), (ii) paraformaldehyde (PFA) 2% for 2 , and (iii) PFA 3.7% for 20 for all the three cell lines. Additionally, for the HEK-293 cell line, two additional fixation methods were added: methanol/C 3 H 6 O (Acetone) and cryofixation.
The advantages and limitations of each preparation method were investigated using low-energy X-ray fluorescence (LEXRF), in conjunction with scanning transmission X-ray microscopy (STXM) and AFM. The advantage of AFM lies in its ability to non-destructively study the morphology of biological samples at the cellular and subcellular level with a spatial resolution in the nanometre range. Therefore, it is an ideal approach to assessing volume and thickness differences in biological samples. In this work, it was used prior to X-ray analyses.

Results
As shown in Figure 1, three different fixation procedures were applied to all samples selected for this study; HEC-1-A endometrial cells, spermatozoa, and the HEK-293 cell line were prepared with three different protocols, i.e., 70% ethanol (EtOH), paraformaldehyde (PFA) 2% for 2 , and PFA 3.7% for 20 . For the last cell line, i.e., HEK-293, two additional fixation methods were tested: methanol/C 3 H 6 O and cryofixation. AFM measurements with a spatial resolution of 200 nm were first performed on the different selected cells, which were then analysed by XRFM and STXM. For XRFM, the cells were analysed at 1.5 keV to determine the intracellular distribution and XRF intensities of essential life elements such as Na, Mg, and O; at the same time, absorption and differential phase contrast images were acquired in STXM mode. While XRFM allows for elemental distribution inspection, STXM imaging provides morphological information; absorption images are sensitive to different sample thickness and/or density, and phase contrast images highlight borders or structures. analysed at 1.5 keV to determine the intracellular distribution and XRF intensities of essential life elements such as Na, Mg, and O; at the same time, absorption and differential phase contrast images were acquired in STXM mode. While XRFM allows for elemental distribution inspection, STXM imaging provides morphological information; absorption images are sensitive to different sample thickness and/or density, and phase contrast images highlight borders or structures.
The XRF results were compared with and complemented by the AFM images.  The XRF results were compared with and complemented by the AFM images.

XRFM Analysis
The XRF elemental maps of selected HEC-1-A endometrial cells fixed with the three different protocols, i.e., 70% ethanol (EtOH), paraformaldehyde (PFA) 2% for 2 , and PFA 3.7% for 20 , are shown in Figure 2. Absorption and phase contrast images (STXM) show no significant change in cell morphology with PFA 3.7% for 20 and PFA 2% for 2 protocols. At the same time, a less defined membrane edge is observed with ethanol fixation. Indeed, in the differential phase contrast image (PhC) of Figure 2a, the cells' borders appear more blurred or less sharp for EtOH treatment than in the corresponding PFA 3.7% or PFA 2% fixations (PhC in Figure 2b,c). In Figure 2d, we show the average Na, O, and Mg values extracted from all the XRF maps collected for the three protocols. Compared to the standard PFA of 3.7% for 20 , fixation with PFA of 2% for 2 can result in lower light element content, especially Na and, to a lesser extent, Mg. Fixation with 70% ethanol retains the highest Na levels but results in a deficiency of Mg (Figure 2d). It is worth noting that even if we did not quantify the elements' amount, average XRF counts of oxygen can be selected to compare the different fixation methods in terms of precision index, as shown in Figure 2e. The coefficient of variation was determined to assess the extent of variability relative to the population mean, as it is widely used to express the precision and repeatability of an assay; a higher coefficient of variation (CV) reflects a large dispersion around the mean. Although the mean fluorescence counts (MFC) are not statistically different when considering the uncertainties, PFA 2% has the highest CV (18.37%) compared to EtOH and PFA 3.7%, for which CV was 5.95% and 9.20%, respectively (see Table S1. HEC-1-A descriptive analysis). All in all, fixation with PFA 3.7% for 20 seems to preserve the internal cellular structure and thereby the Na and Mg content in the cells more efficiently (Figure 2d).   (d) Normalised average XRF counts of O, Na, and Mg in HEC-1-A adenocarcinoma endometrial cells fixed with EtOH 70%, PFA 2%, and 3.7% evaluated on at least 6 cells/fixation method. (e) Min-to-max box plot comparing oxygen MFC as obtained by descriptive statistical analysis used to determine the coefficient of variation. A two-way ANOVA with multiple comparisons test was performed to test the statistical difference among the fixation methods. *** p < 0.001. The STXM images (Abs and PhC) and XRF images were acquired at 1500 eV excitation energy with a step size of 200 nm and 800 nm, respectively, and an acquisition time of 10 ms/pixel and 6 s/pixel, respectively.

AFM
AFM microscopy was performed prior to XRF measurements on all cell lines to investigate the effects of the fixation procedure on cell morphology and volume changes. The AFM images of HEC-1-A endometrial cells fixed by the different methods and grown on Si 3 N 4 membranes are shown in Figure 3. The three representative cell groups selected in Figure 2 are shown in the first panels of Figure 3a (EtOH), Figure 3b (PFA 2%), and Figure 3c (PFA 3.7%), together with other cells prepared with the same fixation method not shown in Figure 2 for spatial constraints. The AFM images confirm that there is no significant difference in cell morphology between the PFA 2% and PFA 3.7% protocols. Cells fixed with ethanol ( Figure 3a) appear emptier and less compact, with the membrane edges tending to become less sharp and less defined. This is in agreement with what has been previously highlighted by comparing the differential phase contrast images of Figure 2. Cells in PFA 3.7% have a higher mean volume (264.1 ± 212.3) overall compared to PFA 2% (196.0 ± 104.8) and EtOH 70% (163.3 ± 104.8); although the three values are comparable within their uncertainties, there is a progressive reduction of the cell volume from PFA 3.7% to EtOH.   (Figure 4b) and 3.7% (Figure 4c) does not alter the morphological phenotype of the spermatozoa, which is characterised by a typically oval head and regular shape of the neck, midpiece, and tail. In contrast, when fixed with ethanol 70%, they appear dehydrated, and the tails are strongly curved (Figure 4a). Figure Figure 4e shows the distribution of sperm oxygen levels; in this case, the coefficient of variation for PFA 3.7% (17.14%) is higher than for EtOH 70% (10.51%) and PFA 2% (7.1%), respectively. Spermatozoa XRF data show a trend which can be considered in agreement with that shown for HEC-1-A cells concerning PFA 3.7% preparation. However, a lower reproducibility level is observed, with high values of uncertainties that can be attributed to the peculiar feature of this cell type; indeed, we found a high degree of variability between different donors and sometimes between cells from the same donor (see Table S2. Spermatozoa descriptive analysis). Figure 5 shows the AFM results for the same spermatozoa groups shown in Figure 4.

AFM
The mean values of cell volume are comparable for the PFA 3.7% and PFA 2% fixatives, while a significantly lower volume is calculated for the cells fixed with ethanol ( Figure 5d).

HEK-293 2.3.1. XRFM Analysis
The HEK-293 cell line was also fixed with PFA 2%, 3.7%, and EtOH. Moreover, additional fixation methods were tested on the HEK-293 cell line, as shown in Figure 1 and described in Section 4. All XRF data are summarised in Figure 6. The PFA 3.7% protocol again proves to be a valid preparation method that appropriately preserves all metals and "living elements". Although the ethanol method does not seem effective in preserving the Mg content in the cells, the Na XRF intensity is well-preserved (Figure 6a). Interestingly, the methanol/C 3 H 6 O and cryofixation methods show the highest Mg XRF counts in the cells, followed by PFA 3.7%, while PFA 2% and ethanol favour the loss of Mg XRF intensity. As for Na, methanol/C 3 H 6 O has the highest level, followed by PFA 3.7%, while cryofixation, EtOH, and PFA 2% show acceptable levels, although lower ( Figure 6f). The washing processes increase the depletion of Na and Mg (see Figure S1). It is worth noting that the overall average O XRF counts are less affected by the preparation compared to Na and Mg and can be considered as a reference for comparing the possible Na and Mg depletions among the different fixation methods. From the absorption images and elemental distribution maps, it is possible to appreciate how fixation with ethanol and 3.7% PFA give similar results, while the absorption image of the cell fixed with 2% PFA is blurred, indicating partial degradation of the sample. Although the Na and Mg XRF intensity seems to be less affected by methanol/C 3 H 6 O and cryofixation, Figure 6d shows how methanol/ C 3 H 6 O fixation increases the precipitation of Na aggregates on the cells, which is visible in both the absorption and phase contrast images and even more so in the Na-XRF map; this is probably due to a reaction between the solvent and the PBS buffer used to wash the cells. This artefact accounts for the highest value of Na for methanol/C 3 H 6 O fixed cells. Cells that have been fixed with methanol/ C 3 H 6 O and then washed do not show the same Na clusters ( Figure S1), but the cells appear to be "depleted", and the total amounts of O, Na, and Mg decrease significantly. Similar considerations apply when comparing ethanol fixation with the same fixation followed by subsequent washing (see Supplementary Materials). The PFA 2% protocol achieves similar results to the ethanol protocol concerning the O, Na, and Mg XRF counts, but the absorption and phase contrast images clearly show impaired cell morphology. The coefficient of variation of oxygen, used as the dispersion parameter of the XRF measurement, changes between the different methods, with very high values for the cryofixed cells and the ethanol-treated cells. At the same time, the other protocols give relatively low values of CV (see Table S3. HEK-293 descriptive analysis).  Figure 4e shows the distribution of sperm oxygen levels; in this case, the coefficient of variation for PFA 3.7% (17.14%) is higher than for EtOH 70% (10.51%) and PFA 2% (7.1%), respectively. Spermatozoa XRF data show a trend which can be considered in agreement with that shown for HEC-1-A cells concerning PFA 3.7% preparation. However, a lower reproducibility level is observed, with high values of uncertainties that can be attributed to the peculiar feature of this cell type; indeed, we found a high degree of variability between different donors and sometimes between cells from the same donor (see Table S2. Spermatozoa descriptive analysis).   Figure 5 shows the AFM results for the same spermatozoa groups shown in Figure  4. The mean values of cell volume are comparable for the PFA 3.7% and PFA 2% fixatives, while a significantly lower volume is calculated for the cells fixed with ethanol ( Figure  5d).

XRFM Analysis
The HEK-293 cell line was also fixed with PFA 2%, 3.7%, and EtOH. Moreover, additional fixation methods were tested on the HEK-293 cell line, as shown in Figure 1 and described in Section 4. All XRF data are summarised in Figure 6. The PFA 3.7% protocol again proves to be a valid preparation method that appropriately preserves all metals and "living elements". Although the ethanol method does not seem effective in preserving the Mg content in the cells, the Na XRF intensity is well-preserved (Figure 6a). Interestingly, the methanol/C3H6O and cryofixation methods show the highest Mg XRF counts in the cells, followed by PFA 3.7%, while PFA 2% and ethanol favour the loss of Mg XRF intensity. As for Na, methanol/C3H6O has the highest level, followed by PFA 3.7%, while cryofixation, EtOH, and PFA 2% show acceptable levels, although lower (Figure 6f). The washing processes increase the depletion of Na and Mg (see Figure S1). It is worth noting that the overall average O XRF counts are less affected by the preparation compared to Na and Mg and can be considered as a reference for comparing the possible Na and Mg depletions among the different fixation methods. From the absorption images and elemental distribution maps, it is possible to appreciate how fixation with ethanol and 3.7% PFA give similar results, while the absorption image of the cell fixed with 2% PFA is blurred, indicating partial degradation of the sample. Although the Na and Mg XRF

AFM
Interestingly, AFM images of methanol/C 3 H 6 O preparation (Figure 7d) show that the morphology of HEK-293 cells is significantly altered, with submicrometric features appearing like clumps on their surface. As mentioned earlier, according to the XRF maps, these features appear to be closely associated with Na nanoclusters. When prepared with ethanol (Figure 7a), the morphology is better preserved, although the cells appear somewhat depleted. This is even more pronounced in the cells fixed with PFA 2% (Figure 7b), as their overall height appears reduced compared to methanol and ethanol fixation; moreover, the cells prepared with PFA 2% have visible nanometric holes on their surface, clearly indicating some stress. In contrast, cells prepared with PFA 3.7% (Figure 7c) appear more filled, as evidenced by their height, and have a smoother surface; overall, they appear healthier and with a better-preserved morphology. AFM images with corresponding surface profiles collected on a selection of (a) 1:1 MeOH/C 3 H 6 O washed cells and of (b) 70% ethanol washed cells are reported in Supporting Materials in Figure S2. absorption and phase contrast images clearly show impaired cell morphology. The coefficient of variation of oxygen, used as the dispersion parameter of the XRF measurement, changes between the different methods, with very high values for the cryofixed cells and the ethanol-treated cells. At the same time, the other protocols give relatively low values of CV (see Table S3. HEK-293 descriptive analysis).    Figure 6), while the other columns depict additional cells prepared with the same five fixation methods. * p < 0.05, ** p < 0.005, *** p < 0.001, **** p < 0.0005.

Discussion
XRF analysis is a powerful, non-destructive, analytical technique with wide application in biomedical science, allowing the chemical characterisation, with good detection limit and high spatial resolution, of trace elements that may play an essential role in cellular biochemical processes. We have recently presented some important results on cells derived from reproductive tissues, observing Na, Cu, and Mg distribution in spermatozoa [21] and ovarian tissues [22]. In another work, we also demonstrated that it is possible to merge compositional and morphological information to quantitatively derive the element concentration by combining XRFM with AFM and STXM analyses [23]. The faithfulness of XRF measurements is highly dependent on the proper preparation of the samples, which is indeed a critical step in obtaining the appropriate information; it requires careful attention in order to preserve the cellular morphology and the elemental localisation inside the cells.
The present study illustrates the effect of several cell fixation methods in singlecell analyses on the localisation and intracellular levels of light elements by synchrotron radiation XRF. As already reported, the most affected elements are the most diffusible ones, namely the light ones, such as Na, Mg, K, Cl, and Ca [15,16]. However, in the available literature, there is a lack of a comprehensive evaluation of the morphological changes correlated to elemental preservation or possible losses after fixation.
We focused on analysing the impact of preparation techniques on the determination of "life elements" O, Na, and Mg inside the cells, using the TwinMic soft X-ray microscope, which also allows for morphological investigations through high-resolution (sub-micrometric length scale) absorption and phase contrast images [23]. Even if the concentration of intracellular elements inside the cells cannot be represented by XRF counts nor MFC parameter alone, the present study aims at illustrating the effect of different fixation methods on cell morphology and elemental distribution. Oxygen XRF counts can be used as a reference to compare Na and Mg changes, while AFM microscopy performed prior to X-ray analyses indeed enabled us to examine at nanometric resolution the changes in cell volumes and morphology induced by the different fixation methods.
In order to provide a more systematic and comprehensive understanding, we decided to compare different fixation protocols on three cell models. Cell fixation methods were chosen accordingly to the following motives: (i) cross-linker, (ii) organic solvent, and (iii) frozen methods. Usually, chemical fixation preserves structures in a state (both chemically and structurally) as close to living tissue as possible by stabilising the proteins, nucleic acids, and other macromolecules. For instance, PFA 3.7% fixation is among the most used for X-ray microscopy and immune-and histochemistry analyses, having the ability to permeabilise cells, in addition to a quick fixation period. Different chemical fixatives are characterised by different permeabilisation grades, reflecting anomalous elemental diffusion from the cells. For this reason, we tested a few examples of chemical fixatives: PFA 3.7%, PFA 2%, ethanol 70%, and 1:1 methanol/ C 3 H 6 O. While the first three methods were applied to all cell models, methanol/ C 3 H 6 O and cryofixation were used only for the HEK-293 cells, which are highly reproducible, thus allowing for a more comprehensive analysis.
Our results confirm that the PFA 3.7% protocol is an excellent compromise to preserve both morphological features, including cell volume, and light element content to a reasonable extent. The findings align with Perrin et al. [15], confirming that Na XRF intensity is well-preserved in PFA 3.7% treated cells and even better for the MeOH/C 3 H 6 O protocol. However, when investigating at a submicrometric length scale, our results demonstrate that the high Na levels after methanol fixation are due to nanometric Na agglomerates or precipitates onto the cells ( Figure S1), thus excluding this fixative since it introduces evident artefacts. Moreover, our results evidence that the fixations with organic solvents greatly affect the morphology or the volume, probably due to their dehydrating effect.
While we still observe significant Mg levels for both PFA 3.7% and MeOH/C 3 H 6 O fixations, for Perrin et al. [15] its elemental content seems to be reduced below the detection limits in both cases. PFA 2% does not show any advantage compared to PFA 3.7%, as the cells treated with this method usually present a lower cell volume and a lower XRF counts of Mg. Furthermore, we compared those results with ethanol fixation, which is a frequently used protocol, highlighting good preservation of Na levels, but not of Mg and cellular volume. All the observations mentioned above concerning PFA 3.7%, PFA 2%, and ethanol effects on elemental XRF intensities, and thus on elemental content, are substantially confirmed in all cell models used in this study (Figures 2-7), providing a good consistency to our results. However, AFM analyses revealed that the way PFA 2% affects the three cell models differs in terms of cell volume, with HEC-1-A endometrial cells the least affected ( Figure 3). Spermatozoa cells show the highest variability in cell volume modifications when fixed with PFA 2%, suggesting that the cell dimension, which in this case is highly variable, may affect the final deformation. The maximal effect for the HEK-293 embryonic line is likely due to their undifferentiated phenotype, as seen in Figure 7b, where the PFA 2% fixed cells seem to collapse and cover a wider surface. In addition, they present irregular cellular profiles. Hence, too mild of a treatment with PFA is insufficient to cross-link the structural cell component, thus resulting in rapid degradation.
Our data with HEK-293 cells suggest cryofixation as the best method, as it ensures the highest cell volume, very likely the closest to the physiological one. Moreover, in agreement with Perrin et al. [15], it maintains a high level of Mg while inducing a moderate loss of Na ( Figure 6e). However, cryofixation with freeze-drying is a sensitive step because biological samples usually contain a high percentage of water. If not properly performed, it can lead to elemental redistribution, loss of elements, shrinking of the specimens, and severe morphology distortion [24].
Cryofixation provides the most truthful representation of the cellular biological structure; however, a limit is the lower repeatability compared to other protocols, as shown by the measurement of the oxygen coefficient of variation (Figure 6g). This is probably due to an intrinsic technical difficulty of operating in a standardised way [25]. To summarise, PFA fixation at 3.7% is the recommended protocol in the absence of cryofixation, even though our results and other ones from literature [15,16,26] suggest that all chemical fixatives affect some aspects of the measurement.
Finally, attention must be paid to water washing after fixation since our results demonstrate that it has some influence on elemental XRF counts, as organic fixatives are known to perforate cell membranes, inducing a release of elemental content outside the cell.
The main analytical constraints of the methods under study are summarised in Table 1 according to our study and the literature [15,16,26]. To note, the study was performed on a limited population of cells due to two main factors: (i) access to a synchrotron facility is granted only for scientific merit, assessed by a peer review process carried out every 6 months; (ii) low-energy XRF is not an efficient phenomenon, as below 2 keV the Auger effect is the dominant process, which results in a low florescence yield and thus long measurement times. Despite these intrinsic limitations, the reported results still provide very useful information to the X-ray microscopy and XRF 3.
1:1 MeOH/C 3 H 6 O for 3 min at −20 • C Then all membranes were washed twice in PBS and twice in distilled water and air-dried.

5.
Cryofixation: cells were washed with ammonium acetate buffer solution 100 mM pH 7.4 prepared with high purity water (Fisher Scientific™ Accu100 Ultrapure Water System), the excess washing buffer was removed, and then Si 3 N 4 membranes were rinsed in ethane (−160 • C) by using a home-made machine; cells were subsequently freeze-dried by leaving the specimens overnight in a controlled pressure system, allowing the ice to sublimate and slowly reach atmospheric pressure and temperature.
All reagents used for fixation are highly pure ones bought from Sigma Aldrich-Merck (Milano, Italy) (PFA 158127, Ethanol 32221, PBS P4417). The PFA was also filtered with a 0.2 micron filter prior to use to eliminate aggregate samples.

AFM Microscopy
The AFM measurements were performed at the NanoInnovation Laboratory located at Elettra-Sincrotrone Trieste (Trieste, Italy). Suitable cells, prepared as described in Section 4.1, were selected through visible light microscopy and then mapped with AFM microscopy prior to XRF analysis. This was done in order to avoid any possible artefacts caused by radiation damage induced by soft X-rays. AFM micrographs were acquired in contact mode in air with an XE100 (Park Instruments) or a MFP3D (Asylume Research/Oxford Instruments) instrument. For the acquisition of images, we used soft cantilevers (Mikromasch CSC38, radius of curvature <10 nm, spring constant 0.006 N/m) at a 0.1-0.2 Hz scanning rate and a 80-160 nm pixel resolution. Images were analysed with Gwyddion software [28]; volume extraction was carried out by flattening the image to remove background, selecting the cells by a height-threshold based mask, and measuring the zero-basis volume of the single cells. Graphs of AFM trace profiles were obtained using the Igor Pro software (Wavemetrics, Lake Oswego, OR, USA).

XRF Microscopy
The XRF measurements were performed at the TwinMic beamline of Elettra-Sincrotrone Trieste (Trieste, Italy) [29]. The TwinMic microscope was operated in scanning transmission mode (STXM), where the specimen is raster-scanned across a microprobe delivered by a zone plate diffractive optic. The transmitted photons are collected through an X-ray-visible light converting system by a fast readout CCD camera providing absorption and differential phase contrast images [30]. Simultaneously, the XRF emitted by the sample is collected by eight SDDs located symmetrically in front of the sample [31,32]. The sample plane is located perpendicularly to the beam axis and the measurements are conducted at room temperature and in high vacuum condition. For the present experiment, an incident energy of 1.5 keV was chosen for optimal excitation of Na and Mg, allowing the detection of O as well. The zone plate optic (600 µm in diameter with an outermost zone width of 50 nm and a central stop of 140 µm) was focusing the incident X-ray photons on the sample on a spot size of 200 nm to 1 µm in diameter, according to the analysed sample and the incident beam intensity available during the experiments. The collected XRF spectra were deconvolved with the PyMCA software package [33]. For endometrial cells, at least three areas were mapped per fixation type, for a total of six analysed cells/fixation method, while for the HEK-293 cell line, at least four cells were mapped per fixation protocols. As far as for the sperm cells, for each of the three donors, a range of six to ten were analysed for each type of fixation.
The presented XRF counts and the relative MFC were calculated as average values on the whole cell.
A comparison about the microscopies used in the manuscript and a summary of a few experimental details are given in Table S5. Please note that in the table we consider generic applications of those microscopies, but we acknowledge that special ones exist as